Ursolic acid (purity, >90%) was purchased from Sigma-Aldrich (Aldrich U6753; Shanghai, China). The total protein extraction and TRIzol total RNA extraction kits were purchased from Invitrogen (Carlsbad, CA, USA). Anti-phospho-IκBα (anti-pIκBα; phospho-S32/S36; sc-8404), anti-NF-κBp65 (sc-8008), anti-Bcl-2 (sc-509) and anti-caspase-3 (sc-7272) antibodies were purchased from Santa Cruz Biotechnology, Inc. (Santa Cruz, CA, USA). Anti-phospho-Akt1 (anti-pAkt1; phospho-T308; ab105731) and anti-glyceraldehyde 3-phosphate dehydrogenase (anti-GAPDH; ab8245) monoclonal mouse antibodies were obtained from Abcam (Beijing, China). Horseradish peroxidase (HRP)-labeled goat anti-mouse secondary antibody was purchased from Abcam. 3-(4,5-dimethylthiazol-2-yl)2,5-diphenyltetrazolium bromide (MTT) was purchased from Sigma (St. Louis, MO, USA). The Moloney Murine Leukemia Virus Reverse Transcriptase (M-MLV RTase) kit was purchased from Promega (Beijing, China). The 2X SYBR real-time PCR kit was obtained from Roche (Shanghai, China). The bicinchoninic acid (BCA) protein detection kit and the enhanced chemiluminescence (ECL) detection kit were purchased from Pierce Chemicals, Thermo Fisher Scientific Inc. (Rockford, IL, USA).

The T24 human urinary bladder cancer (transitional cell carcinoma) cell line was purchased from the American Type Culture Collection (ATCC; no. HTB-4; Manassas, VA, USA). The cells were cultured in Dulbecco’s modified Eagle’s medium (DMEM) containing 10% fetal bovine serum (FBS) (Invitrogen, Gibco, Carlsbad, CA, USA) in a 5% CO₂ incubator and were passaged with a 0.25% trypsin (Sigma)/0.03% EDTA solution.

T24 cells were digested, suspended and seeded in each well of 6-well plates at a density of 1.0×10⁶/ml in 2 ml of complete culture medium. The cells were cultured for 24 h and exposed to ursolic acid for 48 h. Ursolic acid was dissolved in anhydrous ethanol, then added to the cells at final concentrations of 12.5, 25 or 50 μmol/l. An equivalent amount of ethanol was added to the cells as a control.

T24 cells were harvested and total RNA was extracted with the total RNA extraction kit using the TRIzol method. First-strand cDNA was synthesized using M-MLV RTase according to the manufacturer’s instructions and real-time PCR was performed using the cDNA template according to the manufacturer’s instructions. The amplification of GAPDH was used as an internal control in each reaction system. The reaction conditions were as follows: 40 cycles of 95°C for 30 sec, 58°C for 60 sec and 72°C for 60 sec. The primers were designed based on the GenBank sequence using Beacon Designer 7 (Premier Biosoft, Palo Alto, CA, USA) and the primer sequences were verified using Blast (26). Primer synthesis and DNA sequencing were performed by Shanghai Sangon Biotechnology (Shanghai, China). The primer sequences were as follows: NF-κBp65 sense, 5′-GCAAAGGAAACGCCAGAAGC-3′ and antisense, 5′-CACTACCGAACATGCCTCCAC-3′; Bcl-2 sense, 5′-ATGACTTCTCTCGTCGCTACT-3′ and antisense, 5′-CCCATCCCTGAAGAGTTCCGA-3′; caspase-3 sense, 5′-CATGGCCTGTCAGAAAATAC-3′ and antisense, 5′-TAACCCGAGTAAGAATGTGC-3′; and GAPDH (housekeeping gene) sense, 5′-AATGTGTCCGTCGTGGATCTG-3′ and antisense, 5′-CAACCTGGTCCTCAGTGTAGC-3′.

Western blotting was used to detect the protein expression levels of pAkt1, pIκBα, NF-κBp65, Bcl-2 and caspase-3. The T24 cells were harvested and cell lysis was performed using the eukaryotic cell lysis buffer according to the manufacturer’s instructions, followed by extraction of the total protein. Protein quantity was determined using the BCA method. For each sample (30 μg), proteins were separated by 12% SDS-PAGE and blotted with a wet transfer device (BioRad Laboratories, Inc., Shanghai, China) onto nitrocellulose membranes. The membranes were then immersed in a blocking solution containing 10% skimmed milk in PBS Tween-20 (PBST), followed by agitation for 1 h. After washing three times with Tris-buffered saline Tween-20 (TBST) for 5 min each time, the membranes were immersed in the primary antibody at a dilution of 1:1,000 with the blocking solution at room temperature and then agitated for 1 h. After washing, the membranes were incubated in the HRP-labeled secondary antibody at a dilution of 1:10,000 with the blocking solution at room temperature and then agitated for 1 h. After an additional rinse, the membranes underwent color development using the ECL method, followed by X-film photography. GAPDH protein was used as an internal control. The grayscale values (total raw density) of blots were measured using the VisionWorksLS analysis software available in the UVP EC3 (600) Imaging System (Ultra-Violet Products, Upland, CA, USA).

The medium was refreshed to discard the ursolic acid. The cells were supplemented with 20 μl MTT solution (5 mg/ml), followed by incubation in a CO₂ incubator for 4 h. The supernatant was discarded and 100 μl dimethylsulfoxide (DMSO; Sigma) was applied to each well. When the purple crystals at the bottom of the well were completely dissolved, the absorbance value was measured with a Thermo Multiskan MK3 microplate reader (Thermo Fisher Scientific Inc., Waltham, MA, USA) at a wavelength of λ=490 nm. Cell viability (%) was calculated as experimental absorbance/normal absorbance × 100.

Data are expressed as the mean ± standard deviation (SD). The statistical software SPSS10.0 was used for statistical analysis. Paired comparisons were performed using the Student’s t-test. P<0.05 was considered to indicate a statistically significant difference.

The expression of cell signaling molecules detected using qPCR are shown in Fig. 1. Prior to ursolic acid treatment, the control cells expressed high mRNA levels of anti-apoptotic NF-κBp65 and Bcl-2 and a low level of pro-apoptotic caspase-3 mRNA. As increasing concentrations of ursolic acid were applied (12.5, 25.0 and 50.0 μmol/l), the anti-apoptotic signaling was inhibited and pro-apoptotic signaling was activated. Anti-apoptotic NF-κBp65 levels decreased 0.74 (38.9/52.6), 0.35 (18.6/52.6) and 0.17 (8.9/52.6)-fold, respectively; and Bcl-2 levels decreased 0.77 (32.6/42.3), 0.50 (21.3/42.3) and 0.22 (9.5/42.3)-fold, respectively. Pro-apoptotic caspase-3 levels increased 1.63 (13.2/8.1), 2.53 (20.5/8.1), 4.78 (38.7/8.1)-fold, respectively. The pro-apoptotic induction triggered by ursolic acid occurred in a dose-dependent manner.

Fig. 2 shows the expression of the cell signaling molecules, detected using western blotting. Prior to treatment with ursolic acid, high levels of anti-apoptotic pAkt1, pIκBα, NF-κBp65 and Bcl-2 and low levels of pro-apoptotic caspase-3 were expressed in the control cells. With the application of increasing concentrations of ursolic acid (12.5, 25.0 and 50.0 μmol/l), all the anti-apoptotic signaling was inhibited (Fig. 2A), while the pro-apoptotic signaling was upregulated (Fig. 2B).

Table I shows the complete grayscales of the blots presented in Fig. 2, demonstrating the total levels of the proteins detected. The blot grayscales for the anti-apoptotic pAkt1 protein were 26.6, 10.4 and 5.1 vs. 32.3; for pIκBα were 17.3, 8.8 and 3.2 vs. 24.2; for pNF-κBp65 were 32.2, 21.2 and 8.5 vs. 45.1; for Bcl-2 were 33.6, 19.7 and 9.2 vs. 40.3; and for pro-apoptotic caspase-3 protein were 6.1, 11.6 and 20.7 vs. 4.7, respectively (12.5, 25.0 and 50.0 μmol/l ursolic acid vs. control). The pro-apoptotic induction triggered by ursolic acid treatment occurred in a dose-dependent manner.

Fig. 3 shows the cell viability after 48 h of treatment with ursolic acid. The proliferative activity of T24 cells treated with 12.5, 25.0 and 50.0 μmol/l ursolic acid decreased and was significantly lower compared with that of the control cells (83.8, 56.2, 31.5 vs. 97.6%, respectively; P<0.05 for each). The antitumor effect of ursolic acid treatment occurred in a dose-dependant manner.